Cortistatin Is Expressed in a Distinct Subset of Cortical Interneurons

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Volume 17, Number 15, Issue of August 1, 1997 pp. 5868-5880
Copyright ©1997 Society for Neuroscience

Cortistatin Is Expressed in a Distinct Subset of Cortical Interneurons

Luis de Lecea¹, José Antonio del Rio³, José R. Criado², Soledad Alcántara³, Marisela Morales², Patria E. Danielson¹, Steven J. Henriksen², Eduardo Soriano³, and J. Gregor Sutcliffe¹
Departments of ¹ Molecular Biology and ² Neuropharmacology, The Scripps Research Institute, La Jolla, California 92037, and ³ Unitat de Biologia Cel.lular, Facultat de Biologia, Universitat de Barcelona, Barcelona, 08028 Spain

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

Cortistatin is a presumptive neuropeptide that shares 11 of its 14 amino acids with somatostatin. In contrast to somatostatin,administration of cortistatin into the rat brain ventricles specificallyenhances slow wave sleep, apparently by antagonizing the effectsof acetylcholine on cortical excitability. Here we show that preprocortistatinmRNA is expressed in a subset of GABAergic cells in the cortexand hippocampus that partially overlap with those containing somatostatin.A significant percentage of cortistatin-positive neurons is alsopositive for parvalbumin. In contrast, no colocalization was foundbetween cortistatin and calretinin, cholecystokinin, or vasoactiveintestinal peptide. During development there is a transient increasein cortistatin-expressing cells in the second postnatal week inall cortical areas and in the dentate gyrus. A transient expressionof preprocortistatin mRNA in the hilar region at P16 is paralleledby electrophysiological changes in dentate granule cells. Together,these observations suggest mechanisms by which cortistatin mayregulate cortical activity.
Key words: cortistatin; preprocortistatin; mRNA; slow wave sleep; GABAergic stimulation; somatostatin

INTRODUCTION

We recently isolated a cDNA clone of the rat mRNA encoding preprocortistatin, the putative 112 amino acid precursor of a novelneuropeptide structurally related to somatostatin (de Lecea etal., 1996). Cortistatin shares 11 of 14 residues with somatostatin,including those that are known to be responsible for somatostatinbinding to its receptors (Veber et al., 1979) and the cysteinesthat are likely to render the peptide cyclic. The cDNA sequenceand chromosomal localization of cortistatin and somatostatin indicateclearly that they are the products of separate genes (de Leceaet al., 1996, 1997). Synthetic cortistatin was shown to shareseveral biological properties with somatostatin (de Lecea et al.,1996), but its effects on cortical electrical activity and sleepwere distinct from those found for somatostatin. Moreover, cortistatinwas shown to antagonize the effects of acetylcholine on corticalmeasures of excitability, whereas somatostatin enhances acetylcholinerelease and potentiates acetylcholine responses (Mancillas etal., 1986; Araujo et al., 1990). These observations demonstratedthat cortistatin is functionally distinct from somatostatin andraised the possibility that cortistatin exerts its activitiesvia an uncharacterized cortistatin-selective receptor, althoughother explanations of different functionalities can be considered.

Preliminary in situ hybridization studies to determine the anatomical locations of the cells that produce preprocortistatindetected scattered cells throughout the cortex and hippocampus.The positions of these cells in relation to pyramidal cells ofthe hippocampus suggested that they were inhibitory interneurons,a hypothesis consistent with the electrophysiological findings(de Lecea et al., 1996). The complex population of intrinsic inhibitoryGABAergic neurons in the cortex and hippocampus has been subgroupedby its specific afferent connectivity and the presence of calcium-bindingproteins (calbindin, parvalbumin, and calretinin; de Felipe, 1993;Cauli et al., 1997; Kondo et al., 1997) and neuropeptides [cholecystokinin(CCK), Hendry and Jones (1985); vasoactive intestinal peptide(VIP), Morrison et al. (1984); neuropeptide Y (NPY) and somatostatin(SST), Hendry et al. (1984a), Schmechel et al. (1984), Somogyiet al. (1984), and Freund and Buzsáki (1996)]. Calbindin-containingcortical interneurons are also positive for several neuropeptidesand are known to make somatodendritic contacts with pyramidalcells (Gulyás and Freund, 1996). On the other hand, parvalbuminis expressed in a nonoverlapping set of fast-firing interneuronsthat make GABAergic synapses on cell bodies and axon initial segmentsof projection cells (Celio, 1986; Kawaguchi and Hama, 1987; deLecea et al., 1995). The distribution of calretinin partiallyoverlaps with calbindin and labels additional GABAergic cells(Jacobowitz and Winsky, 1991; Miettinen et al., 1992; Acsádyet al., 1993).

Here we show that the cortistatin-expressing cells of the cortex and hippocampus are GABAergic and positive for calbindinand parvalbumin. We examine the relationships between somatostatin-and cortistatin-containing cells and find that in many areas theyare independent populations, but in some regions there are variableextents of coexpression. We also analyze the appearance of cortistatinmRNA in the cerebral cortex and hippocampus during developmentand use electrophysiological techniques in vivo to correlate functionalchanges with the transient expression of cortistatin in the dentategyrus. These results, together with previous physiological observations,suggest mechanisms by which cortistatin may regulate corticalactivity.

MATERIALS AND METHODS
In situ hybridization. We conducted in situ hybridization essentially as described elsewhere (de Lecea et al., 1994) withminor modifications. Briefly, Sprague Dawley rats at various developmentalstages (P0, P5, P10, P12, P16, P21, and adults) were anesthetizedand perfused intracardially with 4% paraformaldehyde (PF) in PBS,pH 7.4. Brains were removed and post-fixed in the same fixativeovernight and cryoprotected in sucrose dissolved in 4% PF. Thenbrains were frozen, and sections 25 µm thick were collected incryoprotectant solution (30% glycerol, 30% ethylene glycol, and0.1 M PBS). Free-floating sections were incubated in 0.1% TritonX-100 in PBS, deproteinized with 0.1N HCl for 10 min, acetylatedwith acetic anhydride (0.25% in 0.1 M triethanolamine hydrochloride,pH 8), post-fixed for 10 min in 4% PF, and prehybridized at 55°Cfor 3 hr in a solution containing 6× PIPES, 10% (w/v) dextransulfate, 50% formamide, 5× Denhardt's, 40 mM DTT, 100 µg/ml yeastRNA, and 100 µg/ml denatured salmon sperm DNA. We labeled a cortistatinriboprobe by in vitro transcription of a 128 bp fragment (nucleotides310-438) encoding rat cortistatin, using T3 polymerase (Ambion,Austin, TX) and ³⁵S-uridine 5 $'$ -triphosphate (UTP) (DuPont NEN, Boston, MA). Labeledantisense cRNA was added to the sections (10⁷ cpm/ml) and incubated overnight at 55°C. Sections were transferredto new vials and washed with 2× SSC, 10 mM $beta$ -mercaptoethanol ( $beta$ -ME)(room temperature for 10 min), digested with RNase A (37°C for1 hr), and washed again with 1× SSC, 50% formamide, 5 mM $beta$ -ME(55°C for 1 hr), and 0.1× SSC plus 0.1% Sarkosyl (30 min, 68°C).Sections were mounted on coated slides (Fisher Scientific, Houston,TX) and exposed to x-ray film and later to Ilford K5 autoradiographicemulsion for 4 weeks at 4°C. We developed the slides with KodakD19 and counterstained with Richardson's blue. A sense cRNA probe,transcribed with T7 RNA polymerase, was included as a negativecontrol for most hybridization experiments.

Double-label in situ hybridization. We labeled the two isoforms of rat glutamic acid decarboxylase (GAD 65 and GAD 67, generouslyprovided by Dr. Allan Tobin, University of California Los Angeles,Los Angeles, CA) with digoxigenin (DIG; Boehringer Mannheim, Indianapolis,IN) and T3 RNA polymerase by in vitro transcription, as describedby the manufacturer. We pretreated the tissue as described aboveand added 10⁷ cpm/ml ³⁵S-labeled cortistatin and 200 ng of DIG-labeled GAD65 or GAD67.After being washed at high stringency, sections were incubatedwith an alkaline phosphatase-conjugated antibody to DIG (1:5000;Boehringer Mannheim) and developed with nitroblue tetrazoliumand 5-bromo-4-chloro-3-indolyl phosphate (BCIP) alkaline phosphatasesubstrates (Life Technologies, Gaithersburg, MD). We then mountedthe sections and dipped them in emulsion, as described above.

Combined immunohistochemistry with in situ hybridization. To detect both protein and mRNA in the same sections, we conductedin situ hybridization first and then incubated the sections withprimary antibodies for 12 hr at 4°C, as described (Alcántaraet al., 1996). After washing the sections with PBS, we incubatedwith biotinylated secondary antibodies and ABC-peroxidase (VectorLaboratories, Burlingame, CA). We used 0.5 mg/ml diaminobenzidine(filtered through 0.22 µm; Sigma, St. Louis, MO) and 0.01% H₂O₂as peroxidase substrates. Then sections were mounted and dippedin emulsion. Calbindin-specific (1:2000), calretinin-specific(1:2000), and parvalbumin-specific (1:3000) antibodies were obtainedfrom SWant (Bellinzona, Switzerland). Antisera to VIP (1:500),CCK (1:1000), or somatostatin (1:2000) have been characterizedelsewhere (Morrison et al., 1983). The antibody to somatostatin(S328) recognizes the N-terminal region of somatostatin-28 andtherefore is unlikely to cross-react with cortistatin.

Data analysis. Sections were examined with a Zeiss Axiophot microscope (Oberkochen, Germany). The delimitation of regionaland laminar boundaries was performed according to Zilles (1985).For the quantitative analysis of labeled neurons, only sectionsprocessed in parallel under exactly the same conditions and displayingsimilar background levels (<10 grains/100 µm²) were considered. Because the autoradiographic background levelswere less than six grains per cell, neuronal somata were consideredpositive when overlaid by 15 or more silver grains, although positiveneurons normally displayed >25 grains. Sections hybridized witha sense riboprobe never exceeded the background threshold. Twodifferent animals were analyzed for each age. To determine theradial distribution of cortistatin mRNA-positive cells, we harvestedeight vertical strips (250 µm wide) covering the entire corticalthickness in the following areas: somatosensory (first parietalarea, PAR1), motor (hindlimb-forelimb, HL-FL), and visual (primarymonobinocular, occipital, OC1M-B) cortices and hippocampal CA1.The number of labeled cells in single layers was counted and theirpercentage relative to the remaining cortical laminae calculated.For quantitative analysis of double-labeled neurons, the numbersof immunoreactive cells displaying positive and negative hybridizationin the somatosensory cortex were counted in 6-15 sections fromtwo to three animals for each neurochemical marker. Densitiesof cortistatin-expressing cells were determined by counting positivecells in eight frames (650 × 440 µm) corresponding to the somatosensoryand visual areas of three different animals.

Northern blot. Cytoplasmic RNA from whole brain samples of Sprague Dawley rats at various developmental stages (except E14,in which the whole head was homogenized) was extracted as described(Schibler et al., 1980). Two micrograms of poly(A⁺) RNA were run on agarose formaldehyde gels, transferred to nylonmembranes, and hybridized with a ³²P-labeled cortistatin probe. Cyclophilin was used as a controlprobe for loading and RNA integrity (Danielson et al., 1988).

Electrophysiology. Male Sprague Dawley rats (adult group: 280-300 gm, 50-60 d old; P15 group: 27-31 gm, 15-17 d old) wereanesthetized with halothane (3-4%) and placed into a stereotaxicapparatus. Halothane was adjusted to 0.7-0.9% on completion ofsurgery and maintained at that level throughout the duration ofthe experiment. Body temperature was measured and maintained at37°C ± 0.5°C by a feedback-regulated heating pad. Evoked fieldpotentials were recorded by one-barrel micropipette (3.0 M NaClfilled; 6-11 m $Omega$ ; 1-2 µm, i.d.) glued to a four-barrel iontophoresiselectrode (tip extending 10 µm ahead of the multibarrel tip) stereotaxicallyoriented into the dentate gyrus (coordinates: 2.5-3.5 mm posteriorand 2.0-2.5 mm lateral to bregma; 2.4-3.0 mm ventral from dura).Acquisition, analysis, and processing of data on- and off-linewere performed by customized National Instruments LabVIEW softwareon Macintosh computers. Square-wave constant pulses (0.2-1.4 mA;0.15 msec duration) were generated by a Grass PSIU6 isolationunit controlled by a MASTER 8 pulse generator. Population spikes(PS) were elicited in the dentate gyrus by stimulation of theangular bundle of the perforant path (coordinates: 6.0-8.1 mmposterior and 4.0-4.2 mm lateral from bregma; 2.5-3.5 mm ventralfrom dura) with insulated, bipolar stainless steel electrodes.Paired-pulse curves were tested by administering two stimuli withvarying interstimulus intervals (10-260 msec) at half-maximumstimulus intensity. The PS amplitude evoked by the second stimuluswas expressed as a percentage of the first. Cortistatin (1 mg/ml)was dissolved in saline and administered iontophoretically throughone barrel of a multibarreled micropipette with Medical Systems(Greenvale, NY) IP-2 iontophoresis pumps and BH-2 balance unit.We routinely used retention (backing) currents of 5-15 nA andautomated balance in the side NaCl barrel to reduce polarizationartifacts. Cortistatin was ejected by positive currents (50-150nA) and retained with negative currents. Results of experimentalgroups from calculations performed on the stimulus-response andpaired-pulse data were expressed as mean ± SEM. Results were comparedby repeated measures or completely randomized design ANOVA.

RESULTS

Distribution of cortistatin-positive cells
We used in situ hybridization to analyze the expression of preprocortistatin mRNA in adult rat brain. Film autoradiographyof coronal sections showed a discrete and punctate pattern throughoutthe cerebral cortex and hippocampus, possibly corresponding tosingle neurons. Weak hybridization labeling was observed in thestriatum and olfactory bulb, but no signals could be detectedin the thalamus, midbrain, cerebellum, or spinal cord. Of note,signals were also absent from hypothalamus, an important siteof somatostatin expression.

We examined the sections by emulsion autoradiography. The cerebral cortex was the area of the brain that contained the mostcortistatin-positive cells. In the neocortex cortistatin mRNA-expressingneurons were found in all cortical areas and layers, except inlayer I (Fig. 1A,B). In all cortical regions cortistatin-positiveneurons were most abundant in layers II-III and VI (Fig. 2). Therewere also clear differences in the number of positive cells andintensity of hybridization in different cortical areas. The visual/temporalcortex displayed approximately twice as many cortistatin-positivecells as other areas, especially in the upper layers (294 ± 8cells/mm² in visual cortex; 162 ± 6 cells/mm² in somatosensory cortex; Figs. 1A-C, 2).
Fig. 1. Cortistatin expression in the adult cortex. A, Dark-field view of a coronal section of the rat visual cortex hybridized witha cortistatin riboprobe. Very heavy labeling was observed in thedeep layers, whereas in the upper layers both the number of positivecells and their cortistatin mRNA concentration were lower. B,The bright-field image of A. C, In situ hybridization of preprocortistatinmRNA in the somatosensory cortex. Note that there are substantiallyfewer cells in the upper layers, as compared with A. D, Dark-fieldmicrograph of a coronal section across the hippocampal formation,which includes the granule cell layer of the dentate gyrus. Somelabeling was found in the CA1 field (arrows), especially in thestratum oriens (so), although some neurons in the pyramidal celllayer (sp) and stratum radiatum (sr) also could be detected. Veryfew or no labeled cells were found in the dentate gyrus (dg).E, Bright-field view of D. Scale bar, 100 µm.
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Fig. 2. Camera lucida drawings showing the distribution of cortistatin mRNA in coronal sections of the cerebral cortex of adult ratsat three different rostrocaudal levels. Each dot represents threelabeled cells. Cg, Cingulate cortex; Ent, entorhinal cortex; Fr,frontal cortex; FL, forelimb area; HP, hippocampus; Oc1, occipitalcortex, area 1; Oc2, occipital cortex, area 2; Par1, parietalcortex, area 1; Par2, parietal cortex, area 2; Pir, piriform cortex;PRh, perirhinal cortex; RS, retrosplenial cortex; Te1, temporalcortex, area 1; Te3, temporal cortex, area 3; I-VI, cortical layers.Scale bar, 1 mm.
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Cortistatin-positive neurons were present in layer III of the piriform cortex as well as in layers III-IV of the entorhinalarea. In the hippocampal region cortistatin mRNA-expressing neuronswere scattered through the subiculum and CA1 region, where theywere concentrated in the stratum oriens and to a lesser extentin the pyramidal layer (Fig. 1D,E). Cortistatin-positive cellswere present in the CA3 region at low density (fewer than fivecells per section). In the adult, hybridization signals were virtuallyabsent from the hilus, but a few neurons (two to three cells persection) could be detected in the granule cell layer (Fig. 1D,E).

Other areas of the brain also showed cortistatin hybridization, although at lower intensity. In the olfactory bulb, granuleGABAergic neurons were heavily labeled with autoradiographic silvergrains. In the striatum a small number of positive cells resemblingcholinergic or GABAergic interneurons displayed very low levelsof hybridization. A few cells in the periventricular hypothalamicnucleus, which were detected only with very long exposures ofemulsion autoradiography, were positive for cortistatin mRNA.No signals were detected in the thalamus, mesencephalon, brainstem,cerebellum, or spinal cord.

Cortistatin is expressed exclusively in GABAergic interneurons
The above pattern of localization suggested that cortistatin mRNA might be present in a subset of GABAergic nonpyramidal interneurons.To confirm the GABAergic nature of cortistatin-expressing cells,we used double in situ hybridization for cortistatin and GAD65/GAD67mRNAs. We labeled a rat cortistatin riboprobe with ³⁵S-UTP and the rat GAD65 and GAD67 probes with DIG. In both theneocortex and hippocampus (Fig. 3A) all cortistatin-positive cellswere also positive for GAD65 or GAD67. More cortistatin-labeledcells were positive for GAD65 (77%) than for GAD67 (40%) in allcortical layers, probably reflecting the ratio of GAD65/67 expressionin the neocortex. These results suggest that most, if not all,cortistatin-positive cells are GABAergic.
Fig. 3. Colocalization of preprocortistatin mRNA with different markers of cortical interneurons. A, Cortistatin-positive cells (clustersof silver grains) overlap with digoxigenin-labeled GAD65- positivecells (arrows). B, In the upper layers of the neocortex, cortistatin-positivecells (filled arrow) do not overlap with somatostatin-immunoreactivecells (open arrow). C, The dentate gyrus, which is abundant insomatostatin immunoreactivity (open arrows), contains very fewcortistatin-expressing cells that are localized in the granulecell layer (filled arrow); h, hilar region; gcl, granule celllayer. D, A significant number of cortistatin-positive cells wasalso positive for parvalbumin immunoreactivity in the visual cortex(double-positive cells are marked by thin arrows). E, CortistatinmRNA frequently colocalized with calbindin-immunoreactive material,especially in the deep layers of the visual neocortex (double-positivecells are marked by thin arrows). A cortistatin-only positivecell is marked with a thick arrow. F, In the hippocampus cortistatinmRNA was present in a subset of parvalbumin-positive interneurons(thin arrow); so, stratum oriens; sp, stratum pyramidale. Scalebar, 50 µm.
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Cortistatin and somatostatin label different populations of interneurons
Somatostatin also is expressed by GABAergic interneurons (Kosaka et al., 1988; Esclápez and Houser, 1995). To compare thedistributions of cortistatin and somatostatin, we combined immunocytochemicalstaining for somatostatin with in situ hybridization for preprocortistatin.Strikingly, the two statins exhibited similar radial patternsof distribution being concentrated in layers II-III and VI. However,fewer than one-half of the cortistatin-positive neurons (42%,visual cortex; 33%, somatosensory cortex) displayed somatostatinimmunoreactivity. Conversely, one-fourth (23% in somatosensorycortex; 28% in visual cortex) of somatostatin-immunoreactive neuronsdisplayed cortistatin hybridization signals, demonstrating thatcortistatin and somatostatin are expressed in different populationsof neurons (Figs. 3B, 4A). There were also notable differencesin the degree of colocalization among the cortical layers. Forinstance, in layer II-III and IV most positive neurons expressedeither somatostatin or cortistatin but not both, whereas in deepcortical layers (especially in layer VI) as many as 44% of cortistatin-positivecells also contained somatostatin-like immunoreactivity (Fig.4).
Fig. 4. Preprocortistatin mRNA labels a distinct population of interneurons. A, Layer distribution in the somatosensory cortex ofcortistatin mRNA-positive cells, as compared with somatostatinneurons. The overlap between somatostatin and cortistatin cellsis expressed as the percentage of cortistatin cells that are positivefor somatostatin immunoreactivity and the fraction of somatostatin-immunoreactivecells that also express cortistatin. The number of double-positivecells is indicated to the right of each bar. B, Comparison ofthe distribution of somatostatin and preprocortistatin mRNA-positivecells in the hippocampal CA1 (so, stratum oriens; sp, stratumpyramidale) and hilar region (hilus) of the fascia dentata. Apopulation of cortistatin-positive cells overlaps with parvalbuminboth in the somatosensory cortex (C) and in the hippocampus (D).E, The overlap between calbindin immunoreactivity and cortistatinmRNA-positive cells in the neocortex, as expressed by the percentageof cortistatin cells that are positive for the calbindin antibody.
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In the hippocampal CA1 field 58% of cortistatin-positive cells were also immunoreactive for somatostatin. However, cortistatin/somatostatin-positivecells represented ~30% of the somatostatin population (Fig. 4B).The subiculum displayed a complex mixture of labeled populations.In contrast, only very rarely could we detect the presence ofcortistatin mRNA in the hilar region of adult animals, which wasrich in somatostatin-positive cells (Fig. 3C). These findingsshow that cortistatin and somatostatin are expressed in different,although partially overlapping, populations of cortical interneurons.

Cellular characterization of cortistatin neurons
To characterize further the types of cortical interneurons that expressed cortistatin, we used combined in situ hybridizationfor preprocortistatin mRNA with immunocytochemistry to the calcium-bindingproteins parvalbumin, calbindin, and calretinin and to two neuropeptides.Together, these proteins are known to define several subpopulationsof cortical interneurons (Freund and Buzsáki, 1996). CortistatinmRNA colocalized frequently with parvalbumin, especially in layersII-III of the visual and somatosensory cortices (73%; Fig. 3D)and in the pyramidal layer of the CA1 hippocampal field (75%;Fig. 3F). Double-labeled cortistatin/parvalbumin-positive neuronsrepresented ~40% of the entire population of parvalbumin-immunoreactiveneurons (Fig. 4C,D).

In the deep layers of the cortex 47% of cortistatin mRNA-expressing neurons were labeled with calbindin antibodies, whereasin the supragranular layers and in the hippocampus colocalizationwas rare. The double-labeled slides immunoreacted for calbindin,which labels faintly most pyramidal and granule cells in corticallayers II-III and IV and in the hippocampus, also confirmed thatthese principal neurons did not express cortistatin mRNA (Fig.3E). We rarely detected double-labeled neurons immunoreactivefor calretinin. Finally, cortical interneurons immunoreactivefor CCK or VIP did not express cortistatin mRNA (data not shown).These findings show that cortistatin is expressed in a subsetof calbindin- and parvalbumin-positive interneurons.

Developmental pattern of preprocortistatin mRNA accumulation
We examined the pattern of accumulation of cortistatin mRNA during development. By Northern blot a single 600 nucleotide band,corresponding to preprocortistatin mRNA, accumulated postnatallybetween P5 and P10, achieved its maximal levels by P15, and thendecayed slightly into adulthood (Fig. 5). In situ hybridizationshowed cortistatin-positive cells in the lower levels of the cerebralcortex and the stratum oriens of the hippocampus as early as P0,the earliest time point analyzed (Figs. 5, 6, 7). Stronger hybridizationsignals could be detected at this stage in the cingulate cortexand in the induseum griseum, taenia tecta, and subiculum (Fig.6A,B). At P5 both the number of cortistatin mRNA-expressing cellsand the individual intensity of labeling were increased in theneocortex, although the distribution of labeled cells remainedthe same, with most positive neurons being concentrated in infragranularlayers. A conspicuous increase in cortistatin expression was notedin the hippocampus, which now showed many intensely labeled neuronsin both the stratum oriens and pyramidal layer (Fig. 7).
Fig. 5. Preprocortistatin mRNA accumulation during development. A, Northern blot of mRNAs extracted from whole brain at differenttime points during rat development, hybridized with a cortistatinprobe. The E14 sample was obtained from whole head. An arrow indicatesthe length (as determined by interpolation with unshown markers)of the band that hybridized with the cortistatin cDNA probe, consistentwith that reported for preprocortistatin mRNA (de Lecea et al.,1996, 1997). A cyclophilin probe was hybridized to the same blotas a control for RNA integrity and loading. B, Horizontal sectionsof an in situ hybridization to P10 and P12 rats showing that theincrease in cortistatin signal is attributable to an increasein both the number of positive cells and in the concentrationper cell.
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Fig. 6. In situ hybridization of preprocortistatin mRNA in postnatal animals. A, Film autoradiograph of a coronal section of a P0rat hybridized with a cortistatin riboprobe. Strong hybridizationcan be observed in the subiculum and CA1 region. B, Dark-fieldin situ hybridization of a coronal section of a P0 cortex. Veryfaint neurons were detected in the deep layers (arrows). Dark-field(C) and bright-field (D) micrographs of a P5 temporal cortex areshown. The hybridization levels were low to moderate and confinedto the deep layers of the neocortex. E, Bright-field image ofan in situ hybridization of a P16 parietal cortex. Note the veryhigh levels of hybridization per cell, which are visible evenat low power. The number of positive cells at this age was approximatelythree times that found in adult animals. F, Bright-field micrographof a coronal section through the hippocampal formation of a P16rat. Again, very high levels of hybridization could be detectedin the CA1 region, especially in the stratum oriens and pyramidale.Also, a substantial increase in the number of cells in the granulecell layer and hilar region was evident at this age. dg, Dentategyrus.
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Fig. 7. Camera lucida drawings showing the distribution of preprocortistatin mRNA in coronal sections of the cerebral cortex at P0,P5, P10, and P16 at equivalent rostrocaudal levels. Each dot representsthree labeled cells except in the P0 drawing, in which each positivecell is represented by a dot. CP, Cortical plate; HL, hindlimbarea; HP, hippocampus; Par1, parietal cortex, area 1; Par2, parietalcortex, area 2; Pir, piriform cortex; PRh, perirhinal cortex;RS, retrosplenial cortex; I-VI, cortical layers. Cortical areaswere labeled according to Paxinos and Watson (1988). Scale bar,1 mm.
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At P10-P12 the levels of autoradiographic labeling increased further both in the neocortex and hippocampus (Figs. 5B,C, 7).Of note, some cortical areas such as the temporal and parietalcortices exhibited at these stages strong labeling in supragranularlayers II-III and IV in addition to a large number of labeledneurons in the infragranular layers. In the P10-P12 hippocampusthe distribution of cortistatin-positive cells was similar tothat at P5, but at this later age approximately five to six positivecells per section could be detected in the hilar region. Hippocampalcortistatin-positive cells showed intense hybridization signalsat these ages.

At P16-P21 there was a much stronger labeling than at P12, as judged both by the density of silver grains per cell and bythe number of positive cells in all cortical areas (Figs. 6, 7).In the neocortex a nearly uniform pattern of expression was observed,with all cortical areas displaying a large number of positiveneurons in both the deep cortical layers and the supragranularlayers. Also, the number of cortistatin-positive cells in allcortical areas was greater than in the adult (480 ± 23 cells/mm² in P16 vs 263 ± 15 cells/mm² in adult rats; Fig. 6E). In the hippocampus there were more labeledcells at P16 than in both earlier and adult stages (68 ± 7 cells/sectionat P16, as compared with 51 ± 5.3 cells in the adult; Fig. 6F).This was particularly evident in the hilar region, where cortistatin-expressingcells were virtually absent in the adult.

Electrophysiological characterization of cortistatin actions on dentate function during development
Because the expression of cortistatin mRNA in the dentate hilar region was significantly higher at P15 than in the adult,we examined the effects of cortistatin on dentate function duringthese developmental stages. To investigate whether the adult disappearanceof cortistatin mRNA in hilar interneurons could be paralleledby physiological and pharmacological changes in granule cells,we conducted electrophysiological studies in vivo to characterizethe effects of local application of cortistatin on the excitabilityof granule cells and on the efficacy of local inhibitory circuitsin the dentate gyrus. Stimulation of the perforant path evokedfield potentials recorded in the granule cell layer or hilus ofthe dentate gyrus, the wave forms of which consisted of a relativelyfast negative-going PS superimposed on the positive-going fieldEPSP/IPSP complex. Consistent with previous reports (Wilson, 1984;Bekenstein and Lothman, 1991), we observed that PS amplitudesat half-maximal stimulation were significantly lower in P15 thanin adults (p < 0.005; Fig. 8A). Iontophoretic administration ofcortistatin had no significant effect on PS amplitudes in theadult dentate gyrus (p > 0.05; Fig. 8B). This contrasts with ourprevious observation that cortistatin inhibits PS amplitudes inthe adult CA1 (de Lecea et al., 1996). Moreover, cortistatin suppressedPS amplitudes in the dentate gyrus of P15 rats by at least 40%in three of five animals (p < 0.05; Fig. 8A).
Fig. 8. Electrophysiological characterization of cortistatin actions on dentate function during development. A, Population spike (PS)amplitudes elicited in P15 rats (n = 7) were significantly lowerthan in adult rats (n = 6; asterisk represents significance levelsof p < 0.05; ANOVA). B, Iontophoretic administration of cortistatinsignificantly reduced PS amplitudes in P15 rats (n = 5; p < 0.05)but had no effect on PS amplitudes elicited in adult rats (n =6; p > 0.05). C, Stimulation of the perforant path in P15 ratswas characterized by a longer period of early inhibition. Controlpaired-pulse (PP) responses between P15 and adult rats were significantlydifferent at 40, 60, and 80 msec (n = 5; p < 0.05). Administrationof cortistatin had no effect on PP responses in either group (n= 5/group; p > 0.05). D, Representative recordings of wave formsevoked in the dentate gyrus by perforant path stimulation (50%maximum) from an adult rat (1) and a P15 rat (2). The marked facilitatoryPP response at 80 msec recorded from the adult rat (1) contrastswith the PP response elicited in the P15 rat (2). Calibration:5 mV, 10 msec.
[View Larger Version of this Image (14K GIF file)]

Equipotent paired orthodromic stimulation of the perforant path in the adult dentate gyrus elicited a triphasic test/conditioningresponse curve (Fig. 8C). In contrast, the early inhibitory phaseof the paired-pulse response in P15 rats was significantly longer(Fig. 8C). Statistical analyses showed that paired-pulse responsesin adult and P15 rats were significantly different at 40, 60,and 80 msec (p < 0.05; Fig. 8C; representative recordings areshown in Fig. 8D,E). These data are consistent with previous reportsby Liu et al. (1996), suggesting that GABAergic synapses dominatethe synaptic physiology of most immature granule cells. Iontophoreticadministration of cortistatin had no effect on the paired-pulseresponses elicited on either group (p > 0.05; Fig. 8C).

DISCUSSION
We have used a combination of immunocytochemical and in situ hybridization techniques to identify the cell types that expressthe precursor of the neuropeptide cortistatin in adult and developingrat cortex and hippocampus. We have shown that the novel neuropeptidecortistatin is expressed in a subpopulation of cortical GABAergicinterneurons that comprises subsets of calbindin- and parvalbumin-immunoreactivecortical neurons. Preprocortistatin mRNA and somatostatin areexpressed in distinct but partially overlapping populations ofneurons. However, because colchicine was not used in this study,somatostatin-immunoreactive cells could have been under-represented.The percentages and distribution of colocalization among preprocortistatinmRNA, calbindin, and somatostatin suggest that the cells thatare double-positive for cortistatin and calbindin are also positivefor somatostatin. Cortistatin has been shown to bind to at leastsome somatostatin receptors with an affinity similar to that ofsomatostatin itself (de Lecea et al., 1996). Thus, in some cases,cortistatin and somatostatin may be released from different terminalsor they may compete for the same receptors. In addition, a previousstudy in adult rats showed that cysteamine-induced release ofsomatostatin potentiates the response of dentate granule cellsto perforant path stimulation (Takazawa et al., 1994). In contrast,our electrophysiological data showed that iontophoretic administrationof cortistatin had no effect on PS amplitudes in the adult dentategyrus. These data provide indirect evidence for a putative cortistatinreceptor. The lack of effect of cortistatin on PS amplitudes inthe adult dentate gyrus could be attributable to a disparity inbrain size and packing density of neurons in the brains of P15and adult rats. However, the iontophoretic currents and the durationof the application of cortistatin in this study were similar tothe parameters used in our previous study in which cortistatinsuppressed PS amplitudes in the CA1 region of adult rats (de Leceaet al., 1996).

The cells in which most neuropeptides are produced are calbindin-positive (Hendry et al., 1984b; de Felipe, 1993). The calbindin-positivepopulation of cortical interneurons has been considered nonoverlappingwith basket and chandelier cells, which are stained with parvalbuminantibodies. However, a recent report (Alcántara et al., 1996)has determined that as many as 10% of calbindin neurons are alsoimmunoreactive for parvalbumin in the adult rat neocortex. Thus,it is noteworthy that cortistatin is coexpressed with parvalbuminin some cortical and hippocampal interneurons. The extent of colocalizationbetween cortistatin mRNA and parvalbumin (70%) and calbindin (47%)indicates that cortistatin mRNA is localized preferentially inneurons that are double-positive for calbindin and parvalbumin.Hippocampal neurons that contain somatostatin or parvalbumin havebeen well characterized in terms of their electrophysiologicaland anatomical properties (Lacaille et al., 1987; Sik et al.,1995; Freund and Buzsáki, 1996). The presence of preprocortistatinmRNA in a substantial portion of parvalbumin-positive fast-firingcells suggests a possible biphasic mode of action of parvalbumininterneurons: a fast mode that releases GABA and acts on GABA_areceptors on pre- and postsynaptic cells and a slow mode involvingcortistatin release and G-protein signaling. It is possible thatcortistatin regulates principal cells at multiple levels.

In a previous report we showed that cortistatin enhanced slow wave sleep (SWS), whereas somatostatin does not have any effecton SWS but increases rapid eye movement sleep. Also, in contrastto somatostatin, cortistatin antagonizes the effects of acetylcholineon hippocampal and cortical activity (de Lecea et al., 1996).Cortical somatostatin-containing cells are known to receive inputfrom GABAergic and cholinergic projection cells in the basal forebrain(Freund and Meskenaite, 1992) and from serotonergic neurons inthe median raphe (Halasy et al., 1992). Because single interneuronscontact multiple pyramidal cells and can synchronize pyramidalactivity, this afferent specificity has been proposed as a mechanismfor tight control of the output of principal cells (Cobb et al.,1995). Thus, it may be that cholinergic afferents innervate preferentiallycortistatin-containing cells, providing a circuitry for sleeponset. Consistent with this hypothesis is the fact that a substantialproportion of cortistatin-positive cells resides in the deep layersthroughout the cortex. Because most afferent axons to the thalamusoriginate in the deep layers of the cerebral cortex, cortistatinmay be regulating the corticothalamic interactions that originateEEG spindle activity, a type of EEG wave that occurs at the onsetof SWS (Steriade et al., 1993a). Also, because of its anatomicaldistribution and electrophysiological properties, cortistatincould be a major factor in the maintenance and synchronizationof the slow oscillation (<1 Hz), a cortical rhythm that is characterizedby depolarizing episodes of pyramidal and GABAergic cells andaccompanies delta activity (Steriade et al., 1993b).

The developmental expression of preprocortistatin mRNA shows three major features in the cerebral cortex: (1) cortical neuronsexpress cortistatin mRNA after the typical inside-out gradientof cortical maturation (i.e., first in deep layers and later inupper cortical layers) (Raki $c'$ , 1988); (2) preprocortistatin mRNAconcentration is maximal during the second postnatal week; and(3) at P15-P21 the number of labeled neurons was higher than inthe adult, indicating a transient expression at these stages andsubsequent downregulation. These stages also correspond to thematuration of cortical function. It may be of significance thatcortistatin mRNA is most abundant in the visual cortex and thatits peak of expression occurs during the second postnatal week,coincident with eye opening. Previous studies have pointed outthat the maturation of cortical interneurons is simultaneous withthe first appearance of postsynaptic inhibitory potentials andburst-firing responses linked to NMDA receptors (Luhmann and Prince,1991). These changes in physiological responses of developingneurons may be associated with the appearance of specific NMDAreceptor subunits during the second postnatal week (Williams etal., 1993). The transient expression of preprocortistatin mRNAat late postnatal stages in cortical development is similar tothat reported for other neuropeptides such as somatostatin orNPY (Parnavelas and Cavanagh, 1988). Particularly interestingis the transient expression of preprocortistatin mRNA in the dentategyrus. In vivo field recordings showed a high degree of intrinsicinhibition in the dentate of P15 rats. In these animals high-frequencyperforant path stimulation failed to produce long-term potentiationin granule cells, in contrast with our previous reports in adultrats (Criado et al., 1996). Also in contrast to adult rats, iontophoreticapplication of cortistatin in the hilus of P15 rats significantlyreduced the evoked PS amplitudes, suggesting that cortistatinreceptors may be expressed in this area and functional at thisage. However, despite this evidence for expression of preprocortistatinand a cortistatin receptor and the electrophysiological propertiesof dentate granule cells, in the absence of a specific cortistatinantagonist it is not possible to establish a causal relationshipbetween the presence of preprocortistatin mRNA and the depressedstate of granule cells in the second postnatal week.

Nevertheless, these considerations suggest that the developmental expression of cortistatin is a reflection of major changesin the electrical activity of a distinct subset of GABAergic cells.GABAergic stimulation has been shown to regulate the phenotypeof hippocampal interneurons via the action of brain-derived neurotrophicfactor (BDNF) (Marty et al., 1996). The transient increase inpreprocortistatin mRNA expression during the second postnatalweek could be attributable to increased BDNF activity caused byGABAergic stimulation of cortical neurons. In contrast, at laterdevelopmental stages when GABA inhibits BDNF expression (Berningeret al., 1995), cortistatin mRNA concentration is decreased. Thus,in addition to its synchronization properties described in adultanimals, cortistatin may be involved in refining cortical activity,possibly modulating the establishment of synaptic connectionsin the neocortex and hippocampus during development.

FOOTNOTES

Received March 24, 1997; revised May 19, 1997; accepted May 20, 1997.

This work was supported in part by grants from the National Institute of General Medical Sciences and Comisión Interministerialde Ciencia y Tecnología, Spain. We thank Allan Tobin for providingthe rat GAD65 and GAD67 plasmids.

Correspondence should be addressed to Dr. J. Gregor Sutcliffe at the above address.

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Volume 17, Number 15, Issue of August 1, 1997 pp. 5868-5880 Copyright ©1997 Society for Neuroscience

Cortistatin Is Expressed in a Distinct Subset of Cortical Interneurons

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Volume 17, Number 15, Issue of August 1, 1997 pp. 5868-5880
Copyright ©1997 Society for Neuroscience